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本文引用的文献

1
Compacted DNA nanoparticle gene transfer of GDNF to the rat striatum enhances the survival of grafted fetal dopamine neurons.用压缩 DNA 纳米颗粒将 GDNF 基因转染至大鼠纹状体可增强移植的胎鼠多巴胺能神经元的存活。
Cell Transplant. 2009;18(10):1183-96. doi: 10.3727/096368909X12483162196881. Epub 2009 Jun 22.
2
A partial structural and functional rescue of a retinitis pigmentosa model with compacted DNA nanoparticles.使用紧密型DNA纳米颗粒对视网膜色素变性模型进行部分结构和功能挽救。
PLoS One. 2009;4(4):e5290. doi: 10.1371/journal.pone.0005290. Epub 2009 Apr 24.
3
Biocompatibility of amphiphilic diblock copolypeptide hydrogels in the central nervous system.两亲性二嵌段共多肽水凝胶在中枢神经系统中的生物相容性
Biomaterials. 2009 May;30(15):2881-98. doi: 10.1016/j.biomaterials.2009.01.056. Epub 2009 Feb 28.
4
Long-term transgene expression in the central nervous system using DNA nanoparticles.利用DNA纳米颗粒实现中枢神经系统中的长期转基因表达。
Mol Ther. 2009 Apr;17(4):641-50. doi: 10.1038/mt.2009.2. Epub 2009 Feb 17.
5
Whole animal in vivo imaging after transient, nonviral gene delivery to the rat central nervous system.向大鼠中枢神经系统进行短暂的非病毒基因递送后的全动物体内成像。
Mol Ther. 2008 Nov;16(11):1857-64. doi: 10.1038/mt.2008.183. Epub 2008 Aug 26.
6
Efficient non-viral ocular gene transfer with compacted DNA nanoparticles.用压缩 DNA 纳米颗粒进行高效非病毒眼部基因转染。
PLoS One. 2006 Dec 20;1(1):e38. doi: 10.1371/journal.pone.0000038.
7
Noninvasive monitoring of long-term lentiviral vector-mediated gene expression in rodent brain with bioluminescence imaging.利用生物发光成像对啮齿动物大脑中慢病毒载体介导的基因表达进行长期无创监测。
Mol Ther. 2006 Sep;14(3):423-31. doi: 10.1016/j.ymthe.2006.05.007. Epub 2006 Jul 3.
8
Looking and listening to light: the evolution of whole-body photonic imaging.观察与聆听光线:全身光子成像的发展历程
Nat Biotechnol. 2005 Mar;23(3):313-20. doi: 10.1038/nbt1074.
9
Compacted DNA nanoparticles administered to the nasal mucosa of cystic fibrosis subjects are safe and demonstrate partial to complete cystic fibrosis transmembrane regulator reconstitution.给予囊性纤维化受试者鼻粘膜的致密DNA纳米颗粒是安全的,并显示出部分至完全的囊性纤维化跨膜传导调节因子重构。
Hum Gene Ther. 2004 Dec;15(12):1255-69. doi: 10.1089/hum.2004.15.1255.
10
Dissecting tumor maintenance requirements using bioluminescence imaging of cell proliferation in a mouse glioma model.在小鼠胶质瘤模型中利用细胞增殖的生物发光成像剖析肿瘤维持需求。
Nat Med. 2004 Nov;10(11):1257-60. doi: 10.1038/nm1120. Epub 2004 Oct 24.

DNA 纳米颗粒:利用生物发光成像检测大脑中的长期转基因活性。

DNA nanoparticles: detection of long-term transgene activity in brain using bioluminescence imaging.

出版信息

Mol Imaging. 2011 Oct;10(5):327-39. doi: 10.2310/7290.2010.00053. Epub 2011 Apr 27.

DOI:10.2310/7290.2010.00053
PMID:21521549
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3173525/
Abstract

In this study, we used bioluminescence imaging (BLI) to track long-term transgene activity following the transfection of brain cells using a nonviral gene therapy technique. Formulations of deoxyribonucleic acid (DNA) combined with 30-mer lysine polymers (substituted with 10 kDa polyethylene glycol) form nanoparticles that transfect brain cells in vivo and produce transgene activity. Here we show that a single intracerebral injection of these DNA nanoparticles (DNPs) into the rat cortex, striatum, or substantia nigra results in long-term and persistent luciferase transgene activity over an 8- to 11-week period as evaluated by in vivo BLI analysis, and single injections of DNPs into the mouse striatum showed stable luciferase transgene activity for 1 year. Compacted DNPs produced in vivo signals 7- to 34-fold higher than DNA alone. In contrast, ex vivo BLI analysis, which is subject to less signal quenching from surrounding tissues, demonstrated a DNP to DNA alone ratio of 76- to 280-fold. Moreover, the ex vivo BLI analysis confirmed that signals originated from the targeted brain structures. In summary, BLI permits serial analysis of luciferase transgene activity at multiple brain locations following gene transfer with DNPs. Ex vivo analysis may permit more accurate determination of relative activities of gene transfer vectors.

摘要

在这项研究中,我们使用生物发光成像(BLI)来跟踪使用非病毒基因治疗技术转染脑细胞后的长期转基因活性。与 30 个赖氨酸聚合物(用 10 kDa 聚乙二醇取代)结合的脱氧核糖核酸(DNA)制剂形成纳米颗粒,可在体内转染脑细胞并产生转基因活性。在这里,我们展示了将这些 DNA 纳米颗粒(DNP)单次脑内注射到大鼠皮层、纹状体或黑质中,通过体内 BLI 分析评估,可在 8 至 11 周的时间内产生长期和持续的荧光素酶转基因活性,并且将 DNP 单次注射到小鼠纹状体中可稳定地产生荧光素酶转基因活性达 1 年。体内产生的压缩 DNP 产生的信号比单独的 DNA 高 7 至 34 倍。相比之下,离体 BLI 分析受周围组织信号淬灭的影响较小,显示 DNP 与 DNA 之比为 76 至 280 倍。此外,离体 BLI 分析证实信号来源于靶向的大脑结构。总之,BLI 允许在使用 DNP 进行基因转移后对多个大脑部位的荧光素酶转基因活性进行连续分析。离体分析可能更准确地确定基因转移载体的相对活性。